Lauer Iris, Alessandri Stefano, Pokoj Sven, Reuter Andreas, Conti Amedeo, Vieths Stefan, Scheurer Stephan
Division of Allergology, Paul-Ehrlich-Institut, Langen, Germany.
Mol Nutr Food Res. 2008 Nov;52 Suppl 2:S262-71. doi: 10.1002/mnfr.200700426.
Several hazelnut allergens with different clinical relevance and crossreactive properties have been identified and characterized so far. The aim of this study was to develop protocols for producing relatively large amounts of three recombinant hazelnut allergens Cor a 1.04, Cor a 2, and Cor a 8 in a folded and immunologically active form. The availability of well-characterized, pure recombinant allergens will improve diagnostic in vitro tests for food allergy, by allowing a highly sensitive component resolved diagnosis. Depending on the individual hazelnut allergen, protocols for heterologous production - either as fusion or nonfusion protein - were developed to obtain homogenous protein batches. The resulting proteins were purified by a two-step FPLC method and their IgE antibody reactivity was verified. Identity was verified by N-terminal sequencing and MALDI-TOF-MS analysis. Their secondary and tertiary structure was controlled by circular dichroism (CD)-spectroscopy and NMR analysis. Decisions on the strategies for expression and purification of allergens on a large scale were made on a case by case basis: Preparation of rCor a 1.04 and rCor a 2 as fusion proteins in E. coli from inclusion bodies resulted in approximately 10 mg pure protein per liter whereas rCor a 8 expression in yeast as nonfusion protein yielded 30 mg/L.
到目前为止,已经鉴定并表征了几种具有不同临床相关性和交叉反应特性的榛子过敏原。本研究的目的是开发方案,以生产相对大量的三种重组榛子过敏原Cor a 1.04、Cor a 2和Cor a 8,使其具有折叠且具有免疫活性的形式。特性明确的纯重组过敏原的可得性将通过实现高灵敏度的成分分辨诊断,改进食物过敏的体外诊断测试。根据具体的榛子过敏原,开发了作为融合蛋白或非融合蛋白进行异源生产的方案,以获得均一的蛋白批次。通过两步快速蛋白质液相色谱(FPLC)方法纯化所得蛋白质,并验证其与IgE抗体的反应性。通过N端测序和基质辅助激光解吸电离飞行时间质谱(MALDI-TOF-MS)分析验证其同一性。通过圆二色(CD)光谱和核磁共振(NMR)分析控制其二级和三级结构。大规模过敏原表达和纯化策略的决策是根据具体情况做出的:在大肠杆菌中从包涵体制备rCor a 1.04和rCor a 2作为融合蛋白,每升可产生约10 mg纯蛋白,而在酵母中表达rCor a 8作为非融合蛋白,产量为30 mg/L。
